EPA Document #: EPA/600/R-05/054
METHOD 521 DETERMINATION OF NITROSAMINES IN DRINKING
WATER BY SOLID PHASE EXTRACTION AND CAPILLARY
COLUMN GAS CHROMATOGRAPHY WITH LARGE
VOLUME INJECTION AND CHEMICAL IONIZATION
TANDEM MASS SPECTROMETRY (MS/MS)
Version 1.0
September, 2004
J.W. Munch
M.V. Bassett
NATIONAL EXPOSURE RESEARCH LABORATORY
OFFICE OF RESEARCH AND DEVELOPMENT
U.S. ENVIRONMENTAL PROTECTION AGENCY
CINCINNATI, OHIO 45268
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METHOD 521
DETERMINATION OF NITROSAMINES IN DRINKING WATER BY SOLID PHASE
EXTRACTION AND CAPILLARY COLUMN GAS CHROMATOGRAPHY WITH
LARGE VOLUME INJECTION AND CHEMICAL IONIZATION TANDEM MASS
SPECTROMETRY (MS/MS)
1. SCOPE AND APPLICATION
1.1
1.2
This method provides procedures for the determination of nitrosamines in finished
drinking water. The method may be applicable to untreated source waters and other
types of water samples, but it has not been evaluated for these uses. The method is
applicable to nitrosamines that are efficiently partitioned from the water sample onto
a solid phase extraction (SPE) sorbent, and sufficiently volatile and thermally stable
for gas chromatography. The method includes the following compounds:
Analyte
N-Nitrosodimethylamine (NDMA)
N-Nitrosomethylethylamine (NMEA)
N-Nitrosodiethylamine (NDEA)
N-Nitrosodi-n-propylamine (NDPA)
N-Nitrosodi-n-butylamine (NDBA)
N-Nitrosopyrollidine (NPYR)
N-Nitrosopiperidine (NPIP)
Chemical Abstract Services (CAS)
Registry Number
62-75-9
10595-95-6
55-18-5
621-64-7
924-16-3
930-55-2
100-75-4
The Minimum Reporting Level (MRL) is the lowest analyte concentration that meets
Data Quality Objectives (DQOs) that are developed based on the intended use of this
method. The lowest concentration MRL (LCMRL) is a single laboratory
determination of the lowest true concentration for which a future recovery is
expected, with 99 percent confidence, to be between 50 and 150 percent recovery.
Single laboratory LCMRLs for analytes in this method range from 1.2-2.1 ng/L, and
are listed in Table 1. The procedure used to determine LCMRLs is described
elsewhere.1
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1.3 Laboratories using this method are not required to determine LCMRLs for the
method analytes, but must demonstrate that their laboratory MRLs meet the
requirements in Section 9.2.4.
1.4 Detection limit (DL) is defined as the statistically calculated minimum concentration
that can be measured with 99% confidence that the reported value is greater than
zero.2 The DL is compound dependent and is dependent on extraction efficiency,
sample matrix, fortification concentration, and instrument performance.
Determining the DL for analytes in this method is optional (Sect. 9.2.5). DLs for
method analytes range from 0.26-0.66 ng/L, and are listed in Table 1.
1.5 This method should be performed only by or under the supervision of analysts with
experience in solid phase extractions and chemical ionization GC/MS/MS analyses.
2. SUMMARY OF METHOD
Analytes and a surrogate analyte are extracted by passing a 0.5-L water sample through a
solid phase extraction (SPE) cartridge containing 2 g of 80-120 mesh coconut charcoal
(Sect. 7.2.7). The organic compounds are eluted from the solid phase with a small quantity
of methylene chloride.
The methylene chloride extract is dried and concentrated, and an internal standard is
added. The sample components are separated, identified, and measured by injecting an
aliquot of the concentrated extract onto the fused silica capillary column of a GC/MS/MS
system equipped with a large volume injector injector (LVI), and operated in the chemical
ionization (CI) mode. Because the CI reagent gas used (methanol or acetonitrile) produces
a mass spectrum with only one significant ion, identification and quantitation are
performed in the MS/MS mode.
Compounds eluting from the GC column are identified by comparing their product ion
mass spectra and retention times to reference spectra and retention times in a user created
database. Reference spectra and retention times for analytes are obtained by the
measurement of calibration standards under the same conditions used for samples. The
concentration of each identified component is measured by an internal standard procedure,
i.e. relating the product ion response of the analyte to the product ion response of the
compound that is used as an internal standard. A surrogate analyte, whose concentration is
known in every sample, is measured with the same internal standard calibration procedure.
3. DEFINITIONS
3.1 ANALYSIS BATCH — A set of samples analyzed on the same instrument during a
24 hour period that begins and ends with the analysis of the appropriate Continuing
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Calibration Check (CCC) standards. Additional CCCs may be required depending
on the length of the analysis batch and/or the number of Field Samples.
3.2 CALIBRATION STANDARD (CAL) -- A solution prepared from the primary
dilution standard solution or stock standard solutions and the internal standards and
surrogate analytes. The CAL solutions are used to calibrate the instrument response
with respect to analyte concentration.
3.3 COLLISIONALLY ACTIVATED DISSOCIATION (CAD) -- The process of
converting the precursor ion's translational energy into internal energy by collisions
with neutral gas molecules to bring about dissociation into product ions.
3.4 CONTINUING CALIBRATION CHECK (CCC) - A calibration standard
containing one or more method analytes, which is analyzed periodically to verify the
accuracy of the existing calibration for those analytes.
3.5 DETECTION LIMIT (DL) — The minimum concentration of an analyte that can be
identified, measured and reported with 99% confidence that the analyte
concentration is greater than zero. This is a statistical determination (Sect. 9.2.5),
and accurate quantitation is not expected at this level.2
3.6 EXTRACTION BATCH -- A set of up to 20 field samples (not including QC
samples) extracted together by the same person(s) during a work day using the same
lot of solid phase extraction devices and solvents, surrogate solution, and fortifying
solutions. Required QC samples for each extraction batch include: Laboratory
Reagent Blank, Laboratory Fortified Blank, Laboratory Fortified Sample Matrix, and
either a Field Duplicate or Laboratory Fortified Sample Matrix Duplicate.
3.7 FIELD DUPLICATES (FD1 and FD2) -- Two separate samples collected at the
same time and place under identical circumstances, and treated exactly the same
throughout field and laboratory procedures. Analyses of FD1 and FD2 give a
measure of the precision associated with sample collection, preservation, and
storage, as well as with laboratory procedures.
3.8 INTERNAL STANDARD (IS) -- A pure analyte(s) added to a sample, extract, or
standard solution in known amount(s) and used to measure the relative responses of
other method analytes and surrogates that are components of the same solution. The
internal standard must be an analyte that is not a sample component.
3.9 LABORATORY FORTIFIED BLANK (LFB) -- An aliquot of reagent water or other
blank matrix to which known quantities of the method analytes are added in the
laboratory. The LFB is analyzed exactly like a sample, including the use of sample
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preservatives, and its purpose is to determine whether the methodology is in control,
and whether the laboratory is capable of making accurate and precise measurements.
3.10 LABORATORY FORTIFIED SAMPLE MATRIX (LFSM) -- An aliquot of an
environmental sample to which known quantities of the method analytes are added
in the laboratory. The LFSM is analyzed exactly like a sample, and its purpose is to
determine whether the sample matrix contributes bias to the analytical results. The
background concentrations of the analytes in the sample matrix must be determined
in a separate aliquot and the measured values in the LFSM corrected for background
concentrations.
3.11 LABORATORY FORTIFIED SAMPLE MATRIX DUPLICATE (LFSMD) -- A
second aliquot of the Field Sample, or duplicate Field Sample, that is used to prepare
the LFSM. The LFSMD is fortified, extracted and analyzed identically to the
LFSM. The LFSMD is used instead of the Laboratory Duplicate to assess method
precision when the occurrence of target analytes is low.
3.12 LABORATORY REAGENT BLANK (LRB) -- An aliquot of reagent water or other
blank matrix that is treated exactly as a sample, including exposure to all glassware,
equipment, solvents, reagents, internal standards, surrogates, and sample
preservatives that are used with other samples. The LRB is used to determine if
method analytes or other interferences are present in the laboratory environment, the
reagents, or the apparatus.
3.13 LARGE VOLUME INJECTION (LVI) - An injection into a gas chromatograph that
is larger than the typical 1 or 2 |j,L injection used for hot vaporizing injectors. A
specialized injector and autosampler are usually required. The upper limit of the
injection size is dependent upon the instrumentation used, and the exact mechanism
utilized to accommodate the larger solvent volume. The type of LVI described in
this method uses a temperature programmed vaporizing (PTV) injector (Sect. 3.20).
3.14 LOWEST CONCENTRATION MINIMUM REPORTING LEVEL (LCMRL) - The
single laboratory LCMRL is the lowest true concentration for which the future
recovery is predicted to fall, with high confidence (99 percent), between 50 and 150
percent recovery.1
3.15 MATERIAL SAFETY DATA SHEET (MSDS) -- Written information provided by
vendors concerning a chemical's toxicity, health hazards, physical properties, fire,
and reactivity data including storage, spill, and handling precautions.
3.16 MINIMUM REPORTING LEVEL (MRL)-- The minimum concentration that can
be reported as a quantitated value for a target analyte in a sample following analysis.
This defined concentration can be no lower than the concentration of the lowest
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calibration standard for that analyte, and can only be used if acceptable quality
control criteria for the analyte at this concentration are met. A procedure for
verifying a laboratory's MRL is provided in Section 9.2.4.
3.17 PRECURSOR ION — For the purpose of this method, the precursor ion is the
protonated molecule ([M + H]+) of the target analyte. In MS/MS, the precursor ion
is mass selected and fragmented to produce distinctive product ions of smaller mass.
3.18 PRIMARY DILUTION STANDARD SOLUTION (PDS) -- A solution of several
analytes prepared in the laboratory from stock standard solutions and diluted as
needed to prepare calibration solutions and other needed analyte solutions.
3.19 PRODUCT ION — For the purpose of this method, a product ion is one of the
fragment ions produced in MS/MS by collisionally activated dissociation of the
precursor ion.
3.20 PROGRAMMED TEMPERATURE VAPORIZING INJECTOR (PTV) - A GC
injector capable of rapid heating. Typical use of a PTV injector involves introducing
the sample with the injector cool, then rapidly heating it at 100-200 °C per minute to
volatilize the analytes onto the GC column. One advantage of this type of injection
is that thermally labile analytes in a mixture can be transferred to the GC column at a
lower temperature than in conventional hot injections. It is also useful for large
volume injections.
3.21 QUALITY CONTROL SAMPLE (QCS) -- A solution of method analytes of known
concentrations that is obtained from a source external to the laboratory and different
from the source of calibration standards. It is used to check laboratory performance
with externally prepared test materials.
3.22 STOCK STANDARD SOLUTION (SSS) -- A concentrated solution containing one
or more method analytes prepared in the laboratory using assayed reference materials
or purchased from a reputable commercial source.
3.23 SURROGATE ANALYTE (SUR) - A pure analyte, which is extremely unlikely to
be found in any sample, and which is added to a sample aliquot in a known amount
before extraction or other processing, and is measured with the same procedures
used to measure other sample components. The purpose of the SUR is to monitor
method performance with each sample.
4. INTERFERENCES
4.1 During analysis, major contaminant sources are reagents and SPE devices. Analyses
of laboratory reagent blanks provide information about the presence of
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contaminants. Solid phase extraction devices described in this method have two
potential sources of contamination, both the solid phase sorbent and the
polypropylene cartridge that it is packed in. Manufacturers' brands and lot numbers
of SPE materials should be monitored and tracked to ensure that contamination will
not preclude analyte identification and quantitation.
4.2 Nitrosamines may be present in trace amounts in rubber products. The analyst
should be aware that repeated injections from autosampler vials with PTFE
(polytetrafluoroethylene, otherwise known as Teflon®) coated rubber septa may
introduce method analytes into the sample extracts.
4.3 Interfering contamination may occur when a sample containing low concentrations
of compounds is analyzed immediately after a sample containing relatively high
concentrations of compounds. Injection port liners must be replaced as needed
(cleaning and deactivation by the analyst is not recommended). After analysis of a
sample containing high concentrations of compounds, a laboratory reagent blank
should be analyzed to ensure that accurate values are obtained for the next sample.
In the case of automated analysis, the analyst may not be aware of high concentration
samples until after an entire batch is analyzed. In this situation, the analyst should
carefully review data from samples analyzed immediately after high concentration
samples, and reanalyze them if necessary.
4.4 Reagent water must be free of method analytes. Because NDMA and other
nitrosamines can leach from rubber products, rubber components must be avoided in
the reagent water system. Reagent water contamination with NDMA has been
reported in the literature.3 It is strongly recommended that the reagent water system
include an ultraviolet module. Ultraviolet light is capable of destroying trace
amounts of nitrosamines that may be in the water. During the development of this
method, a Millipore Milli-Q A10 system was used. Reagent water may be
successfully stored in glass bottles with PTFE lined screw caps.
5. SAFETY
5.1 The toxicity or carcinogenicity of many of the chemicals used in this method have
not been precisely defined; each chemical should be treated as a potential health
hazard, and exposure to these chemicals should be minimized. Each laboratory is
responsible for maintaining awareness of OSHA regulations regarding safe handling
of chemicals used in this method. Each laboratory should maintain a file of
applicable MSDSs.
5.2 The analytes listed in this method have been classified as known or suspected human
or mammalian carcinogens.4'5 Pure standard materials and stock standard solutions
of these compounds should be handled with suitable protection to skin, eyes, etc.6"8
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6. EQUIPMENT AND SUPPLIES (References to specific brands or catalog numbers are
included for illustration only, and do not imply endorsement of the product.)
6.1 GLASSWARE — All glassware must be meticulously cleaned. This may be
accomplished by washing with detergent and water, rinsing with water, distilled
water, and solvent rinsing or heating (where appropriate) at 400 °C for 2 h in a
muffle furnace. Volumetric glassware should never be heated to the temperatures
obtained in a muffle furnace.
6.2 SAMPLE CONTAINERS -- 1-L, 1-qt, 1-pt or 0.5-L amber glass bottles fitted with
PTFE lined polypropylene screw caps. Amber bottles are highly recommended since
some of the method analytes are very sensitive to light and will degrade upon
exposure. Clear glass bottles may be used only if they are wrapped in foil, or
samples are stored in boxes that prevent exposure to light.
6.3 VIALS — Screw cap or crimp top amber glass autosampler vials with PTFE faced
septa for storing standards and extracts.
6.4 VOLUMETRIC FLASKS - Class A, various sizes used for preparation of
standards.
6.5 MICRO SYRINGES -- Various sizes.
6.6 BALANCE — Analytical, capable of accurately weighing to 0.0001 g.
6.7 DRYING COLUMN — The drying tube should contain about 5 to 7 grams of
anhydrous sodium sulfate to remove residual water from the extract. During method
development, 6-mL glass reaction tubes with PTFE frits (Supelco cat. # 504394 or
equivalent) were used. Any small tube may be used, such as a syringe barrel, a glass
dropper, etc. as long as no particulate sodium sulfate passes through the column into
the extract.
6.8 CONICAL CENTRIFUGE TUBES -- 60 mL, used to collect extract after it is passed
through anhydrous sodium sulfate and prior to concentration to final volume. Other
glassware suitable for this purpose may be used.
6.9 SOLID PHASE EXTRACTION (SPE) APPARATUS
6.9.1 EXTRACTION CARTRIDGES -- 6-mL polypropylene tubes, to be packed
with 1.8 to 2.2 g of coconut charcoal (Sect. 7.2.7.1). Glass tubes are also
available, and may be used. These tubes are not needed if prepacked SPE
cartridges are used (Sect. 7.2.7.2).
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6.9.2 VACUUM EXTRACTION MANIFOLD -- Equipped with flow/vacuum
control (Supelco cat. #57250-U or equivalent). The use of disposable PTFE
liners to prevent cross contamination may be used.
6.9.3 SAMPLE DELIVERY SYSTEM -- Use of a transfer tube system (Supelco
"Visiprep", cat. #57275 or equivalent), which transfers the sample directly
from the sample container to the SPE cartridge, is recommended. Sample
reservoirs, which attach to the cartridge, may be used, although they hold
only a limited volume of sample.
6.9.4 CONICAL CENTRIFUGE TUBES -- 15 mL, or other glassware suitable
for elution of the sample from the cartridge after extraction.
6.9.5 LABORATORY OR ASPIRATOR VACUUM SYSTEM -- Sufficient
capacity to maintain a vacuum of approximately 25 cm (10 in) of mercury.
6.9.6 An automatic or robotic system designed for use with SPE cartridges may
be used if all quality control requirements discussed in Section 9 are met.
Automated systems may use either vacuum or positive pressure to process
samples and solvents through the cartridge. All extraction and elution steps
must be the same as in the manual procedure. Extraction and/or elution
steps may not be changed or omitted to accommodate the use of an
automated system.
6.10 FUSED SILICA CAPILLARY GAS CHROMATOGRAPHY COLUMN - Any
capillary column that provides adequate resolution, capacity, accuracy, and precision
can be used. Medium polarity, low bleed columns are recommended for use with
this method to provide adequate chromatography and minimize column bleed.
Deactivated injection port liners are recommended.
6.10.1. Column - 30 m x 0.25 mm i.d. fused silica capillary column coated with a
1.0 micron bonded film of polyphenylmethylsilicone, (Restek Rtx 5SIL MS
or equivalent).
NOTE: Although other columns maybe used, shorter or thinner film
columns are not recommended for use with ion trap GC/MS/MS systems
because the chromatographic peak widths will be insufficient to obtain a
sufficient number of MS/MS scans during peak elution.
6.11 GAS CHROMATOGRAPH/MASS SPECTROMETER/DATA SYSTEM
(GC/MS/MS/DS)
6.11.1 The GC must be capable of temperature programming and should be
equipped for large volume injection if low detection limits and MRLs are
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required. The data presented in this method in Section 17 were obtained
using 20-|_iL injections.
6.11.2 Deactivated injection port liners should be used, and it is highly
recommended that they be replaced when necessary with a new deactivated
liner. Cleaning and deactivation of injection port liners by the analyst is not
recommended. The frequency of replacement will vary by the type of
instrument used and the type and number of samples analyzed.
In general, packed injection port liners may be useful in performing large
volume injections. The data demonstrated in this method were obtained
with an injection port liner containing a Carbofrit ® (Restek). The
positioning of the Carbofrit ® is specific to the instrument and liner used.
On the Varian 1078 and 1079 injectors, 2.5 cm from the top of the liner is
appropriate.
6.11.3 The tandem mass spectrometer may be either a triple quadrupole or an ion
trap. However, during the method development, only ion trap mass
spectrometers were used. The MS/MS must be capable of chemical
ionization using either methanol or acetonitrile as the reagent gas. The
mass spectrometer must be capable of scanning at a minimum from 40 to
160 daltons with a complete scan cycle time (including scan overhead) of
0.5 sec or less. The scan time must be set so that all analytes have a
minimum of 5 scans across the chromatographic peak, when operated in
MS/MS mode. Seven to ten scans across chromatographic peaks are
strongly recommended.
6.11.4 An interfaced data system is required to acquire, store, reduce, and output
mass spectral data. The computer software should have the capability of
processing stored GC/MS/MS data by recognizing a GC peak within any
given retention time window. The software must also allow integration of
the ion abundance of any specific ion between specified time or scan
number limits, calculation of response factors as defined in Section 10.2.3
or construction of a linear regression calibration curve, and calculation of
analyte concentrations.
7. REAGENTS AND STANDARDS (References to specific brands or catalog numbers are
included for illustration only, and do not imply endorsement of the product.)
7.1 GASES
7.1.1 CARBON DIOXIDE OR LIQUID NITROGEN - Used to cool the injector
for large volume injections.
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7.1.2 HELIUM — Carrier gas, purity as recommended by the GC/MS/MS
manufacturer.
7.1.3 NITROGEN — Ultra High Purity or equivalent, used to concentrate sample
extracts.
7.2 REAGENTS AND SOLVENTS - Reagent grade or better chemicals should be
used. Unless otherwise indicated, it is intended that all reagents shall conform to the
specifications of the Committee on Analytical Reagents of the American Chemical
Society, where such specifications are available. Solvents should be HPLC grade or
better. Other grades may be used, provided it is first determined that the reagent is
of sufficiently high purity to permit its use without lessening the quality of the
determination.
7.2.1 METHANOL (CH3OH, CAS# 67-56-1) - High purity, demonstrated to be
free of analytes and interferences.
7.2.2 ACETONITRILE (CH3CN, CAS#75-05-8) - High purity, demonstrated to
be free of analytes and interferences.
7.2.3 METHYLENE CHLORIDE (Dichloromethane, CH2C12, CAS# 75-09-2) -
High purity, demonstrated to be free of analytes and interferences.
7.2.4 REAGENT WATER — Purified water which does not contain any
measurable quantities of any target analytes or interfering compounds
greater than 1/3 the MRL for each compound of interest. Refer to Section
4.4 for a description of how reagent water was obtained during method
development.
7.2.5 SODIUM SULFATE, ANHYDROUS (Na^, CAS# 7757-82-6) -
Should be Soxhlet extracted with methylene chloride for a minimum of 4 h
or heated to 400 °C for 2 h in a muffle furnace. Store in a tightly sealed
glass container. For the development of this method, a 10 to 60 mesh size
was used. Finer mesh sized particles may slow the filtering process.
7.2.6 SODIUM THIOSULFATE (Na^A CAS# 7772-98-7) - Dechlorinating
agent, used to eliminate residual chlorine in samples.
7.2.7 SOLID PHASE EXTRACTION MATERIAL - The packing needed for
solid phase extraction in this method consists of activated coconut charcoal,
80 to 120 mesh size.
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7.2.7.1 The product used for most of the method development was a
50:50 mix of 80/100 and 100/120 mesh obtained from Anspec of
Ohio (Anspec, part # OV5487S).9 It is recommended that the
charcoal be Soxhlet extracted with methylene chloride for a
minimum of 8 h, then air dried to evaporate the methylene
chloride (keeping the air drying time minimal) and stored in a
tightly sealed container. Pack 1.8 to 2.2 grams of the dry
coconut charcoal in 6-mL polypropylene cartridges, using
20-micron polypropylene frits at the top and bottom of the tubes.
As the tubes are being filled, periodically tap them on a hard
surface to ensure even packing, without voids. Pack the
cartridges just prior to use or store the packed tubes in a tightly
sealed glass container. Glass SPE tubes may also be used as
described in Section 6.9.1.
7.2.7.2 Pre-packed coconut charcoal cartridges (< 100 mesh) were also
used, and are commercially available (Restek cat. # 26032).
7.2.7.3 NOTE: SPE carbon disks (47 mm) were evaluated during
method development, and determined to have insufficient
capacity to retain all of the nitrosamine analytes using a 0.5-L
water sample. Commercial brands of prepacked carbon SPE
cartridges that contained carbon other than coconut charcoal,
such as graphitized carbon, were also found to be unsatisfactory
for this method.
7.3 STANDARD SOLUTIONS - Standard solutions may be prepared from certified,
commercially available solutions or from neat compounds. Compounds used to
prepare solutions must be 96% pure or greater. The weight may be used without
correction for purity to calculate the concentration of the stock standard. Solution
concentrations listed in this section were used to develop this method and are
included as an example. The majority of the method development work was done
with commercially obtained stock standard solutions, which are readily available
from most suppliers of environmental standards (Accustandard, Ultra, Supelco).
7.3.1 ANALYTE STOCK STANDARD SOLUTION - If preparing from neat
material, accurately weigh approximately 25 to 35 mg of pure material to
the nearest 0.1 mg into a tared, 5-mL volumetric flask. Dilute to the mark
with methylene chloride. Repeat for each target analyte. A serial dilution
of these stock standards, made in methylene chloride, maybe needed prior
to making the final methylene chloride or water primary dilution standards.
Alternatively, a stock standard mix of target analytes may be purchased
commercially. For the development of this method, stock standards of
1000 or 2000 i-ig/mL were used to make primary dilution standards.
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7.3.2 ANALYTE PRIMARY DILUTION STANDARD SOLUTION IN
METHYLENE CHLORIDE (MeCl2 PDS) -- The MeCl2 PDS is a mix of all
of the analytes of interest prepared in methylene chloride and used for
calibration standard preparation. Prepare the analyte MeCl2 PDS by dilution
of the target analyte stock standard(s). Add enough of each target stock
standard (or commercial stock standard mix) to a volumetric flask partially
filled with methylene chloride to make the final desired concentration when
filled to the mark with methylene chloride. During method development, a
2.0-|_ig/mL solution was made by diluting a 2000-|_ig/mL stock standard
solution. This PDS has been shown to be stable for at least 6 months when
tightly capped and stored at -15 °C or less and protected from light.
7.3.3 ANALYTE PRIMARY DILUTION STANDARD SOLUTION IN WATER
(Water PDS) — A PDS of the method analytes prepared in water is used to
fortify LFBs or LFSMs prior to extraction. When an MeCl2 PDS (as
prepared in Sect. 7.3.2) was used to fortify the samples, decreased
recoveries for NDMA were observed. This problem was corrected with the
use of a water PDS. To make this PDS, a 5-|_iL volume of a 2000-|_ig/mL
methylene chloride stock standard (Sect. 7.3.1) was added to a 5-mL
volume of reagent water for a 2.0-|_ig/mL water PDS. The water PDS has
been shown to be stable for at least 45 days when tightly capped and stored
at 4 °C, and protected from light. A lower concentration water PDS may be
useful for fortifying water samples at low concentrations. For this method,
a 100-ng/mL water PDS was also made by adding 5 |_iL of a methylene
chloride stock standard into 100 mL of reagent water. All of the data
demonstrated in this method was obtained using the solution prepared as
described above. However, the analyst is permitted to modify the solvent
that this solution is prepared in, as long as it is a water miscible solvent, and
the QC criteria in Section 9 are met.
7.3.4 SURROGATE (SUR) STOCK STANDARD SOLUTION
(N-Nitrosodimethylamine- cL) — It is recommended that this compound be
obtained as a certified stock standard solution rather than neat material.
During the development of this method, a commercially obtained 1000
1-ig/mL stock standard solution was used (Cambridge Isotopes).
7.3.5 SURROGATE PRIMARY DILUTION STANDARD SOLUTION IN
METHYLENE CHLORIDE (SUR MeCl2 PDS)-- The SUR MeCl2 PDS is a
dilution of the SUR stock standard (Sect. 7.3.4) prepared in methylene
chloride and used for calibration standard preparation. Add enough of the
SUR stock standard to a volumetric flask partially filled with methylene
chloride to make a final concentration of 2.0 |_ig/mL when filled to the mark
with methylene chloride.
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7.3.6 SURROGATE PRIMARY DILUTION STANDARD SOLUTION IN
WATER (SUR Water PDS) - A PDS of the surrogate analyte prepared in
water is used to fortify all water samples prior to extraction. See Section
7.3.3 for the reason a water PDS is used. During the development of this
method, a SUR water PDS was made by adding 10 |_iL of a 1000 |_ig/mL
methylene chloride stock standard (Sect. 7.3.4) to a 5-mL volume of reagent
water for a 2.0 |_ig/mL SUR water PDS. This PDS has been shown to be
stable for at least 45 days when tightly capped and stored at 4 °C, and
protected from light. All of the data demonstrated in this method was
obtained using the solution prepared as described above. However, the
analyst is permitted to modify the solvent that this solution is prepared in, as
long as it is a water miscible solvent, and the QC criteria in Section 9 are
met.
7.3.7 INTERNAL STANDARD (IS) STOCK STANDARD SOLUTIONS
7.3.7.1 N-nitrosodi-n-propylamine-d14 (NDPA-dl4) — It is
recommended that this compound be obtained as a certified
stock standard solution rather than neat material. During the
development of this method, a commercially obtained 1000
1-ig/mL stock standard solution was used (Cambridge Isotopes).
7.3.7.2 N-nitrosodiethylamine-d10(NDEA-dlO) (optional)— This is an
optional second internal standard that may be used to quantify
early eluting peaks, since it elutes early in the chromatogram. At
the time of method development this chemical was available
only in neat form from CDN Isotopes. Prepare in methylene
chloride at a suggested concentration of 1000 |_ig/mL. For long
term storage of stock solutions, prepare in deuterated methylene
chloride.
7.3.8 INTERNAL STANDARD PRIMARY DILUTION STANDARD
SOLUTION -- The IS PDS is a dilution of the internal standard stock
(Sect. 7.3.7) prepared in methylene chloride and used to fortify all sample
extracts and calibration standards. Add enough of the internal standard
stock solutions to a volumetric flask partially filled with methylene chloride
to make a final concentration of 1.0 |-ig/mL when filled to the mark with
methylene chloride.
7.3.9 CALIBRATION STANDARDS (CAL) - For an initial calibration curve
over a concentration range of 2 orders of magnitude, a minimum of at least
5 calibration standards are required. Prepare the calibration standards over
the concentration range of interest from dilutions of the methylene chloride
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PDSs (Sect. 7.3.2, 7.3.5, and 7.3.8). The lowest concentration of calibration
standard must be at or below the MRL (Sect. 9.2.4), which will depend on
system sensitivity. The surrogate standard may be added to all the CAL
standards at the same concentration, or at the analyst's discretion, it maybe
varied to create a calibration curve. The calibration standards used for the
development of this method were prepared as described in the following
table. This table serves only as an example, and adjustments may be made
to meet the needs of the laboratory. In this example, the surrogate standard
is calibrated at a single concentration.
PREPARATION OF CALIBRATION (CAL) CURVE STANDARDS
CAL
Level
1
2
3
4
5
6
7
Vol. of 2.0
Hg/mL
Analyte PDS
MeCl2 GiL)
2.5
5.0
10.0
25.0
25.0
50.0
125.0
Vol. of
2.0 |ig/mL
SUR PDS
MeCl2 GiL)
50.0
50.0
50.0
50.0
25.0
25.0
25.0
Vol. of
1.0|ig/mL
IS PDS
GIL)
200.0
200.0
200.0
200.0
100.0
100.0
100.0
Final Vol. of
CAL Std.
(mL)
10.0
10.0
10.0
10.0
5.0
5.0
5.0
Final Cone.
of Analytes
(ng/mL)**
0.50
1.0
2.0
5.0
10.0
20.0
50.0
** Concentration of SUR is 10 ng/mL and concentration of IS is 20 ng/mL.
Concentration is calculated in final volume.
8. SAMPLE COLLECTION, PRESERVATION, AND STORAGE
8.1 SAMPLE COLLECTION — When sampling from a water tap, open the tap and
allow the system to flush until the water temperature has stabilized (usually about
2 min). Adjust the flow to about 500 mL/min and collect samples from the flowing
stream. The sample should nearly fill the bottle, but does not need to be headspace
free. If the dechlorination agent has been added to the bottle prior to sampling
(Sect. 8.2), be careful not to rinse it out during sample collection. Keep samples
sealed from collection time until analysis. When sampling from an open body of
water, fill the sample container with water from a representative area. Sampling
equipment, including automatic samplers, must be free of plastic or rubber tubing,
gaskets, and other parts that may leach interfering analytes into the water sample.
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8.2 SAMPLE DECHLORINATION -- All samples must be dechlorinated at the time of
collection. Add 80-100 mg sodium thiosulfate for each liter of water. The sodium
thiosulfate may be added to the empty sampling bottles before they are transported to
the sampling location. The material must be added as a solid, because aqueous
solutions of sodium thiosulfate added to the bottles in advance of sampling are not
stable and can be ineffective at dechlorinating the sample.
8.3 SAMPLE TRANSPORT AND STORAGE - All samples should be iced during
shipment and must not exceed 10 °C during the first 48 hours. Samples must be
confirmed to be at or below 10 °C when they are received at the laboratory. Samples
stored in the lab must be held at or below 6 °C until extraction, but should not be
frozen. Chemical freeze packs may be used as a substitute for ice, provided that the
required temperatures can be met.
NOTE: Samples that are significantly above 10 °C at the time of collection, may
need to be iced or refrigerated for a period of time, in order to chill them prior to
shipping. This will allow them to be shipped with sufficient ice to meet the above
requirements.
8.4 AQUEOUS SAMPLE AND EXTRACT HOLDING TIMES - Samples must be
extracted within 14 days of collection. Sample extracts maybe stored for up to
28 days after sample extraction, when stored in amber vials at -15 °C or less, and
protected from light.
9. QUALITY CONTROL
9.1 QC requirements include the Initial Demonstration of Capability and ongoing QC
requirements that must be met when preparing and analyzing Field Samples. This
section describes each QC parameter, its required frequency, and the performance
criteria that must be met in order to meet EPA quality objectives. The QC criteria
discussed in the following sections are summarized at the conclusion of the method,
in Section 17, Tables 8 and 9. The QC requirements described here are considered
the minimum acceptable QC criteria. Laboratories are encouraged to institute
additional QC practices to meet their specific needs.
9.1.1 METHOD MODIFICATIONS - The analyst is permitted to modify GC
columns, GC conditions, LVI techniques and CI and MS/MS parameters.
Each time such method modifications are made, the analyst must repeat the
procedures in Section 9.2.
9.2 INITIAL DEMONSTRATION OF CAPABILITY (IDC) - Requirements for the
initial demonstration of laboratory capability are described in the following sections
and summarized in Table 8.
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9.2.1 INITIAL DEMONSTRATION OF LOW SPE EXTRACTION
BACKGROUND AND SYSTEM BACKGROUND - Before any samples
are analyzed, or any time a new lot or brand of solid phase extraction
materials is received from a supplier, it must be demonstrated that a
laboratory reagent blank (LRB) is reasonably free of any contamination that
would prevent the determination of any analyte of concern (Sects. 9.2.1.2
and 9.4).
9.2.1.1 A source of potential contamination is the solid phase extraction
materials which may contain phthalate esters, silicon
compounds, and other contaminants that could interfere with the
determination of method analytes. Although extraction media
are generally made of inert materials, they may still contain
extractable organic material. If the background contamination is
sufficient to prevent accurate and precise measurements, the
condition must be corrected before proceeding with the initial
demonstration.
9.2.1.2 Other sources of background contamination are solvents,
reagents (including reagent water), and glassware. Reagent
water has been shown to be a potential cause of contamination in
the analysis of nitrosamines.3 Background contamination must
be reduced to an acceptable level before proceeding with the IDP
(Sect. 9.2.2). Background from method analytes and
interferences must be < 1/3 the MRL. If background
contamination is an on-going or intermittent issue for any
method analyte, the analyst must not attempt to verify an MRL
less than the mean LRB concentration + 3o, or three times the
mean LRB concentration, whichever is greater.
NOTE: Although quantitative data below the MRL may not be
reliably accurate enough for data reporting, such data are useful
in determining an MRL cut off for analytes that are typically
detected in LRBs. Therefore, blank contamination levels may be
estimated by extrapolation, when the concentration is below the
lowest calibration standard.
9.2.2 INITIAL DEMONSTRATION OF PRECISION (IDP) - Establish an Initial
Calibration following the procedure outlined in Section 10.2. Prepare 4-7
replicate LFBs fortified at 10-20 ng/L, or other mid-range concentration,
using solutions described in Sections 7.3.3 and 7.3.6. Sodium thiosulfate
must be added to these samples as described in Section 8.2. Extract and
analyze these replicates according to the procedure described in Section 11.
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The relative standard deviation (RSD) of the results of the replicate analyses
must be less than or equal to 20% for all method analytes and surrogates.
9.2.3 INITIAL DEMONSTRATION OF ACCURACY (IDA) -- Using the same
set of replicate data generated for Section 9.2.2, calculate average recovery.
The average recovery of the replicate values for all analytes and surrogates
must be within 70-130% of the true value.
9.2.4 MINIMUM REPORTING LEVEL (MRL) CONFIRMATION -- Select a
target concentration for the MRL based on the intended use of the method.
The lowest calibration standard used to establish the Initial Calibration (as
well as the low-level Continuing Calibration Check standard) must be at or
below the concentration of the MRL. Establishing the MRL concentration
too low may cause repeated failure of ongoing QC requirements. Confirm
the MRL following the procedure outlined below. !
9. 2 A.I Fortify, extract, and analyze 7 replicate Laboratory Fortified
Blanks at the proposed MRL concentration. These LFBs must
contain sodium thiosulfate as described in Section 8.2.
Calculate the mean (Mean) and standard deviation for these
replicates. Determine the Half Range for the prediction interval
of results (HRPIR) using the equation below
HRps = 3.963$
where S is the standard deviation, and 3.963 is a constant value
for seven replicates.
9.2.4.2 Confirm that the upper and lower limits for the Prediction
Interval of Result (PIR = Mean ± HRPIR) meet the upper and
lower recovery limits as shown below.
The Upper PIR Limit must be < 150 percent recovery.
Mean + HR?st
< 1 50%
The Lower PIR Limit must be > 50 percent recovery.
Mean - HRfst
Fortified Concentration
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9.2.4.3 The MRL is validated if both the Upper and Lower PIR Limits
meet the criteria described above. If these criteria are not met,
the MRL has been set too low and must be determined again at a
higher concentration.
9.2.5 DL DETERMINATION (optional) - While DL determination is not a
specific requirement of this method, it may be required by various regulatory
bodies associated with compliance monitoring. It is the responsibility of the
laboratory to determine ifDL determination is required based upon the
intended use of the data.
Replicate analyses for this procedure should be done over at least 3 days
(both the sample extraction and the GC/MS/MS analyses should be done
over at least 3 days). Prepare at least 7 replicate LFBs using solutions
described in Section 7.3.3 and 7.3.6, at a concentration estimated to be near
the DL. This concentration maybe estimated by selecting a concentration at
2-5 times the noise level. The DLs in Table 1 were calculated from LFBs
fortified at 1.0 ng/L; however, the appropriate concentration will be
dependent upon the injection technique and the sensitivity of the GC/MS/MS
system used. Sodium thiosulfate must be added to these samples as
described in Section 8.2. Analyze the seven replicates through all steps of
Section 11.
NOTE: If an MRL confirmation data set meets these requirements, a DL
may be calculated from the MRL confirmation data, and no additional
analyses are necessary.
Calculate the DL using the following equation:
^ n _ 1; j. alpha = 0 99)
where:
t( n -1,1 - alpha = 0.99) = Student's t value for the 99% confidence level with
n-1 degrees of freedom
n = number of replicates
S = standard deviation of replicate analyses.
NOTE: Do not subtract blank values when performing DL calculations.
9.3 INITIAL QCS ANALYSIS - As part of, or immediately following the IDC, analyze
a QCS as described in Section 9.11.
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9.4 LABORATORY REAGENT BLANKS (LRB) -- With each extraction batch,
analyze a laboratory reagent blank to determine the background system
contamination. If, within the retention time window of any analyte, the LRB
produces a peak that would prevent the determination of that analyte, determine the
source of contamination and eliminate the interference before processing samples.
Background contamination must be reduced to an acceptable level before
proceeding. Background from method analytes or contaminants that interfere with
the measurement of method analyses must be < 1/3 the MRL. Any time a new batch
of SPE materials is received, or new supplies of other reagents are used, repeat the
demonstration of low background described in Section 9.2.1.
9.5 CONTINUING CALIBRATION CHECK (CCC) - This calibration check is
required at the beginning of each day that samples are analyzed, after every ten field
samples, and at the end of any group of sample analyses. See Section 10.3 for
concentration requirements and acceptance criteria.
9.6 LABORATORY FORTIFIED BLANK (LFB) -- With each extraction batch, extract
and analyze an LFB containing each analyte of concern, using solutions described in
Sections 7.3.3 and 7.3.6, and the dechlorination agent described in Section 8.2. If
more than 20 field samples are included in a batch, analyze an LFB for every
20 samples. The fortified concentration of the LFB must be rotated between low,
medium, and high concentrations from day to day. The low concentration LFB must
be as near as practical to the MRL. Results of LFB analyses corresponding to the
low fortification concentration for an analyte must be within 50-150% of the true
value. Results of LFB analysis from medium and high level concentrations must be
70-130% of the true value for all analytes.
9.7 INTERNAL STANDARDS (IS) -The analyst must monitor the peak area of the IS
in all injections during each analysis day. The IS response (peak area) in any
chromatographic run must not deviate from the response in the most recent CCC by
more than 30%, and must not deviate by more than 50% from the average area
measured during initial analyte calibration. If the IS area in a chromatographic run
does not meet these criteria, inject a second aliquot of that extract.
9.7.1 If the reinjected aliquot produces an acceptable internal standard response,
report results for that aliquot.
9.7.2 If the reinjected extract fails again, the analyst should check the calibration
by reanalyzing the most recently acceptable calibration standard. If the
calibration standard fails the criteria of Section 10.3.3, recalibration is in
order per Section 10.2.3. and 10.2.4. If the calibration standard is
acceptable, extraction of the sample may need to be repeated provided the
sample is still within the holding time. Otherwise, report results obtained
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from the reinjected extract, but annotate as suspect. Alternatively, collect a
new sample and re-analyze.
9.8 SURROGATE RECOVERY -- The surrogate standard is fortified into all calibration
standards, samples, LFBs, LFSMs, LFSMDs, FDs and LRBs. The surrogate is a
means of assessing method performance from extraction to final chromatographic
measurement.
9.8.1 Surrogate recovery criteria are 70-130% of the fortified amount for the
method surrogate. When surrogate recovery from a sample, blank, or CCC
does not meet these criteria, check: (1) calculations to locate possible errors,
(2) standard solutions for degradation, (3) contamination, and
(4) instrument performance. Correct any problems that are identified. If
these steps do not reveal the cause of the problem, reanalyze the extract.
9.8.2 If the extract reanalysis meets the surrogate recovery criterion, report only
data for the reanalyzed extract.
9.8.3 If the extract reanalysis fails the recovery criterion, the analyst should check
the calibration by reanalyzing the most recently acceptable calibration
standard. If the calibration standard fails the criteria of Section 10.3.3,
recalibration is in order per Section 10.2. If the calibration standard is
acceptable, it may be necessary to extract another aliquot of sample if
sample holding time has not been exceeded. If the sample re-extract also
fails the recovery criterion, report all data for that sample as suspect, or
obtain and analyze another sample.
9.9 LABORATORY FORTIFIED SAMPLE MATRIX (LFSM) - Determine that the
sample matrix does not contain materials that adversely affect method performance.
This is accomplished by analyzing replicates of laboratory fortified matrix samples
and ascertaining that the precision, accuracy, and detection limits of analytes are in
the same range as obtained with laboratory fortified blanks. If a variety of different
sample matrices are analyzed regularly, for example, drinking water from
groundwater and surface water sources, LFSM data should be collected for each
matrix. Over time, LFSM data should be documented for all routine sample sources
for the laboratory.
9.9.1 Within each extraction batch, a minimum of one field sample is fortified as
an LFSM for every 20 samples analyzed. The LFSM is prepared by spiking
a sample with an appropriate amount of the fortification solutions described
in Section 7.3.3 and 7.3.6. Select the spiking concentration that is greater
than or equal to the matrix background concentration. Selecting a duplicate
bottle of a sample that has already been analyzed, aids in the selection of
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appropriate spiking levels. If this is not possible, use historical data or
rotate through low, medium and high calibration concentrations to select a
fortifying concentration.
9.9.2 Calculate the percent recovery (R) for each analyte, after correcting the
measured fortified sample concentration, A, for the background
concentration, B, measured in the unfortified sample, i.e.,
c
where C is the fortified concentration. Compare these values to
control limits for LFBs (Sect. 9.6).
9.9.3 Recoveries may exhibit a matrix dependence. For samples fortified at or
above their native concentration, recoveries should range between 70 and
130% for all method analytes. If the accuracy (percent recovery) of any
analyte falls outside the designated range, and the laboratory performance
for that analyte is shown to be in control, the accuracy problem encountered
with the fortified sample is judged to be matrix related, not system related.
The result for that analyte in the unfortified sample is labeled
suspect/matrix to inform the data user that the results are suspect due to
matrix effects.
9.10 FIELD DUPLICATES (FD) -- Within each extraction batch, a minimum of one field
sample must be analyzed in duplicate. If more than 20 samples are extracted in a
batch, analyze a FD for each 20 samples. Duplicate sample analyses serve as a
check on sampling and laboratory precision. If analytes are not routinely observed in
field samples, LFSMDs must be analyzed to substitute for this requirement. Refer to
Section 9.9.1 for guidance on spiking concentrations.
9.10.1 Calculate the relative percent difference (RPD) for duplicate measurements
(FD1 and FD2) as shown below.
RPD- FD1~FD2 .(100)
FD2)/2
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9.10.2 RPDs for FDs and LFSMDs should be < 30%. Greater variability may be
observed for target analytes whose concentrations are within a factor of 2 of
the MRL. In this case, the RPDs should be <50%.
9.11 QUALITY CONTROL SAMPLE (QCS) -- Each time that new PDSs are prepared,
analyze a QCS from an external source. If standards are prepared infrequently,
analyze a QCS at least quarterly. The QCS may be injected as a calibration standard,
or fortified into reagent water and analyzed as an LFB. If the QCS is analyzed as a
calibration check standard, then the acceptance criteria are the same as for the CCC
(Sect. 10.3.3). If the QCS is analyzed as an LFB, then the acceptance criteria are the
same as for an LFB (Sect. 9.6). If measured analyte concentrations are not of
acceptable accuracy, check the entire analytical procedure to locate and correct the
problem.
10. CALIBRATION AND STANDARDIZATION
10.1 Demonstration and documentation of acceptable initial calibration is required before
any samples are analyzed. After initial calibration is successful, a continuing
calibration check is required at the beginning and end of each period in which
analyses are performed, and after every tenth sample.
10.2 INITIAL CALIBRATION
10.2.1 INSTRUMENT SET-UP FOR LIQUID CI GC/MS/MS - The following
description is a suggested sequence of steps for instrument set-up. Because
of differences in instrumentation, it may be desirable or necessary to alter
these steps. However, it is highly recommended that each part of the
instrumental analysis be added in a stepwise fashion, i.e., first verify that
the instrument works in the CI mode, then optimize the LVI, and then
proceed to MS/MS analysis. It is likely that the method will be slightly less
sensitive in the MS/MS mode than in standard MS. However, the use of
MS/MS is required to provide sufficient specificity and minimize false
positive results.
10.2.1.1 Mass calibrate the MS in El mode using FC-43 or the tuning
compound recommended by the MS manufacturer. A manifold
temperature of 150 °C (Varian Saturn 4) is recommended. On
the Varian Saturn 2000, the recommended manifold temperature
is 50 °C, and the recommended trap temperature is 150 °C. On
other instruments, the manufacturer's recommendation for
instrument temperatures should be followed.
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10.2.1.2 Introduce CI reagent (methanol or acetonitrile) into the MS, and
adjust the level of reagent as directed by the MS manufacturer.
10.2.1.3 Set the instrument acquisition parameters as necessary to collect
data in the CI mode. Example parameters are included in Tables
2a and 2b. It is recommended that during initial instrument set-
up, full scan CI data be acquired. The acquisition mass range
should be 40-160 daltons with a total cycle time (including scan
overhead time) of 0.5 sec or less. Cycle time must be adjusted
to measure at least five or more scans during the elution of each
GC peak. Seven to ten scans across each GC peak are
recommended.
NOTE: On ion trap mass spectrometers, the scan time and the
chromatographic peak width may need to be carefully evaluated
to make sure that this requirement is met, because of the
relatively slow scan speed in MS/MS mode.
10.2.1.4 Analyze a high concentration CAL standard (50-100 pg/|_iL) by
injecting 1-2 |j,L into the GC in the splitless mode. The injection
volume selected will depend upon the injector design.
Suggested GC parameters are: injector temperature 250 °C, split
activation time 1 min. A suggested GC oven temperature
program is presented in Table 3.
10.2.1.5 Identify each analyte by its potonated molecular ion (precursor
ion). Example retention times and precursor ions are presented
in Table 4.
10.2.1.6 Optimize the LVI parameters according to the manufacturer's
instructions. Because of the variety of instrumentation available
for LVI, specific instructions are not discussed here. Some
general literature references on LVI using a programmed-
temperature vaporizing injector (PTV) have been cited.10"12
Example parameters for LVI using a 20-|_iL injection and a PTV
injector are given in Table 3. After LVI optimization, compare the
peak areas from the conventional injection in Sect 10.2.1.4 to the
LVI peak areas. For example, the response from a l-|j,L injection
of a 50-pg/|-iL standard should not vary dramatically from a 10-|_iL
injection of a 5-pg/|_iL standard.
10.2.1.7 Create an MS/MS method by selecting a time window around
each analyte, or in the case of closely eluting analytes, around
each pair of analytes. For analyses using ion trap mass
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spectrometers, it is recommended that no more than two
compounds of interest be contained in an MS/MS time window.
Due to multiple scan events in each time window, it may not be
possible to achieve a sufficient number of scans during the
elution of each chromatographic peak. A minimum of 5 scans
must be obtained during the elution of each chromatographic
peak; however, 7-10 are recommended.
10.2.1.8 Set parameters for the formation of product ions from the
precursor ion. An example of these parameters and the values
used to obtain the demonstration data are found in Tables 5a and
5b. The parameters listed in the tables were selected to produce
product ion spectra with approximately 5% of the precursor ion
remaining. Optimal parameters maybe expected to vary from
instrument to instrument.
10.2.1.9 Analyze a standard at a concentration estimated to be in the
middle of the final calibration range. Create a database that
includes the retention times, product ion spectra and quantitation
ion response for each analyte, surrogate and internal standard.
Suggested quantitation ions are listed in Table 4. Do not select
the precursor ion (molecular ion) as the quantitation ion.
CAUTION: When acquiring MS/MS data, GC operating
conditions must be carefully reproduced for each analysis to
provide reproducible retention times. If this is not done, the
correct ions will not be monitored at the appropriate times. As a
precautionary measure, the chromatographic peaks in each
window must not elute too close to the edge of the time window.
As a minimum, there should be at least 5 sec between the edge
of the time window and the beginning of an analyte peak.
10.2.2 CALIBRATION SOLUTIONS -- Prepare a set of calibration solutions as
described in Section 7.3.9. When selecting calibration standard
concentrations, the analyst should be aware that the MRL cannot be less
than the lowest CAL. Use a minimum of 3 standards for a calibration range
of 1 order of magnitude, and at least 5 standards for 2 orders of magnitude.
During method development, typical calibration curves were generated
from CAL standards of either 0.5 to 20 ng/mL (6 points) or 0.5 to 50 ng/mL
(7 points). Data outside of the established calibration range should never be
reported (Sect. 12.1).
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10.2.3 CALIBRATION — Concentrations may be calculated through the use of
average response factor (RF) or through the use of a calibration curve.
Average RF calibrations may only be used if the RF values over the
calibration range are relatively constant. The RFs must be constant enough
to meet the calibration acceptance criteria in Section 10.2.4.
Average RF is determined by calculating the mean RF of each calibration
point.
where:
AX = integrated abundance (peak area) of the quantitation ion
of the analyte.
Ais = integrated abundance (peak area) of the quantitation ion
internal standard.
Qx = quantity of analyte injected in ng or concentration units.
Qis = quantity of internal standard injected in ng or
concentration units.
As an alternative to calculating average RFs, use the GC/MS data system
software to generate a linear regression or quadratic calibration curve. The
analyst may choose whether or not to force zero, or whether weighting
should be employed to obtain a curve that best fits the data. In general,
forcing zero is not recommended. However, in situations where an analyte
is typically detected in LRBs, forcing zero is recommended. Examples of
common GC/MS system calibration curve options are: 1) Ax /Ais vs Qx /Qis
and 2) RF vs A,, /AIS.
1 0.2.4 CALIBRATION ACCEPTANCE CRITERIA -- Acceptance criteria for the
calibration of each analyte is determined by calculating the concentration of
each analyte and surrogate in each of the analyses used to generate the
calibration curve or average RF. Each calibration standard, except the
lowest point, for each analyte should calculate to be 70-130% of its true
value. The lowest point should calculate to be 50-1 50% of its true value. If
these criteria cannot be met, reanalyze the calibration standards, or select an
alternate method of calibration. The data in this method were generated
using both quadratic fits and average RF, depending upon the analyte.
Quadratic fit calibrations should be used with caution, because the non-
linear area of the curve may not be reproducible.
10.3 CONTINUING CALIBRATION CHECK (CCC) - The minimum daily calibration
verification is as follows. Verify the initial calibration at the beginning and end of
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each group of analyses, and after every tenth sample during analyses. (In this
context, a "sample" is considered to be a field sample. LRBs, LFSMs, LFSMDs,
LFBs and CCCs are not counted as samples.) The beginning CCC each day must be
at or near the MRL in order to verify instrument sensitivity prior to any analyses. If
standards have been prepared such that all low CAL points are not in the same CAL
solution, it may be necessary to analyze two CAL solutions to meet this requirement.
Alternatively, it may be cost effective to prepare or obtain a customized standard to
meet this criteria. Subsequent CCCs must alternate between a medium and high
concentration standard.
10.3.1 Inject an aliquot of the appropriate concentration calibration solution and
analyze with the same conditions used during the initial calibration.
10.3.2 Determine that the absolute areas of the quantitation ions of the internal
standards have not changed by more than 30% from the areas measured in
the most recent continuing calibration check, and by more than 50% from
the average areas measured during initial calibration. If either of the IS
areas has changed by more than these amounts, adjustments must be made
to restore system sensitivity. These adjustments may include cleaning of
the MS ion source, or other maintenance as indicated in Section 10.3.4.
Major instrument maintenance requires recalibration. Control charts are
useful aids in documenting system sensitivity changes.
10.3.3 Calculate the concentration of each analyte and surrogate in the check
standard. The calculated amount for each analyte for medium and high level
CCCs must be within 70-130% of the true value. The calculated amount
for the lowest calibration point for each analyte must be within 50-150% of
the true value. If these conditions do not exist, remedial action should be
taken which may require recalibration. Any field sample extracts that have
been analyzed since the last acceptable calibration verification should be
reanalyzed after adequate calibration has been restored, with the following
exception. If the continuing calibration check in the middle or at the
end of an analysis batch fails because the calculated concentration is
>130% of the true value, and field sample extracts showed no detection
of method analytes, non-detects may be reported without re-analysis.
10.3.4 Some possible remedial actions are: maintenance and/or recalibration of the
MS, GC column and injection port maintenance, and preparation of new
CAL standards. This list is not meant to be all inclusive. Major
maintenance such as cleaning the MS, replacing filament assemblies,
replacing the electron multiplier, changing the GC column, etc. require
returning to the initial calibration step (Sect. 10.2). Changes in the GC
injection or column may affect retention times. After maintenance, verify
all retention times before recalibrating.
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11. PROCEDURE
11.1 This procedure may be performed manually or in an automated mode (Sect. 6.9.6)
using a robotic or automatic sample preparation device. If an automatic system is
used to prepare samples, follow the manufacturer's operating instructions, but all
extraction and elution steps must be the same as in the manual procedure.
Extraction and/or elution steps may not be changed or omitted to accommodate the
use of an automated system.
11.2 Important aspects of this analytical procedure include proper preparation of
laboratory glassware and sample containers (Sect. 6.1 and 6.2), as well as sample
collection and storage (Sect. 8). This section details the procedures for sample
preparation, solid phase extraction (SPE) using cartridges, and extract analysis.
11.3 SAMPLE PREPARATION -
11.3.1 Mark the level of the sample on the bottle prior to extraction for later
sample volume determination. The LRB and LFB may be prepared by
filling a 0.5-L sample bottle with reagent water.
11.3.2 All field and QC samples must contain the dechlorinating agent, sodium
thiosulfate, including the LRB and LFB. Verify that field samples were
dechlorinated at the time of collection. Add 40-50 mg of sodium thiosulfate
to the LRB and LFB at this time and swirl until dissolved.
11.3.3 If 1-qt or 1-L sample bottles were used, transfer 500 mL of the sample to a
clean container.
11.3.4 ADDITION OF SURROGATE ANALYTE -- Add an aliquot of the water
SUR Water PDS (Sect. 7.3.6) to all samples and mix by swirling the
sample. Addition of 5.0 |_iL of a 2.0-|_ig/mL water SUR Water PDS to a
500-mL sample will result in a concentration of 20 ng/L.
11.3.5 FORTIFICATION WITH METHOD ANALYES -- If the sample is an LFB,
LFSM, or LFSMD, add the necessary amount of analyte Water PDS
(Sect.7.3.3). Swirl each sample to ensure all components are properly
mixed.
11.3.6 Proceed with sample extraction.
11.4 SPE PROCEDURE — Proper conditioning of the solid phase sorbent can have a
marked effect on method precision and accuracy. This section describes the SPE
procedure using a transfer tube system and SPE manifold as described in Section 6.9.
521-28
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11.4.1 CARTRIDGE CONDITIONING --
11.4.1.1 Fill the cartridge with approximately 3 mL methylene chloride,
turn on the vacuum, and pull the solvent through, aspirating
completely. Repeat once.
11.4.1.2 Fill the cartridge with approximately 3 mL methanol, turn on the
vacuum, and pull the solvent through, aspirating completely.
Repeat once.
11.4.1.3 Fill the cartridge with approximately 3 mL methanol and elute
with vacuum to just above the top frit - not allowing the
cartridge to go dry at the end. From this point forward, do not
allow the cartridge to go dry. Repeat once.
11.4.1.4 Fill the cartridge with approximately 3 mL reagent water, turn
on the vacuum, and pull the water through, repeat 5 times,
without allowing the cartridge to go dry in between washes or at
the end.
11.4.2 SAMPLE EXTRACTION -- Attach a transfer tube from each sample bottle
to each cartridge and then turn on the vacuum. Adjust the vacuum so that
the approximate flow rate is 10 mL/min. After all of the sample has passed
through each SPE cartridge, detach the reservoir and draw air through the
cartridge for 10 minutes at full vacuum. Turn off and release the vacuum.
Proceed immediately with cartridge elution.
11.4.3 CARTRIDGE ELUTION -- Lift the extraction manifold top and insert a
rack with collection tubes into the extraction tank to collect the extracts as
they are eluted from the cartridges. Fill each cartridge with methylene
chloride. Pull enough of the solvent into the cartridge at low vacuum to
soak the sorbent. Turn off the vacuum and vent the system. Allow the
sorbent to soak in methylene chloride for approximately 1 minute. Apply a
low vacuum and pull the methylene chloride through the cartridge in a
dropwise fashion into the collection tube. Continue to add methylene
chloride to the cartridge as it is being drawn through until the volume of
extract is about 12 or 13 mL, determined by the markings on the side of the
collection tube.
11.4.4 Small amounts of residual water from the sample container and the SPE
cartridge may form an immiscible layer with the extract. To eliminate
residual water, pass the extract through the drying column (Sect. 6.7). The
drying column is packed with approximately 5 to 7 grams of anhydrous
sodium sulfate, and is pre-wetted with a small volume of methylene
521-29
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chloride prior to passing the extract through it. Collect the dried extract in a
clean centrifuge tube (Sect. 6.8). After passing the extract through the
drying tube, wash the sodium sulfate with at least 3 mL methylene chloride
and collect the solvent wash in the same collection tube. Concentrate the
extract to approximately 0.9 mL in a water bath near room temperature
(20 to 25 °C) under a gentle stream of nitrogen. It is strongly recommended
that you do not concentrate the extract to less than 0.5 mL, as this may
result in loss of analytes. Add the internal standard (Sect. 7.3.8). Adjust
final volume to 1.0 mL with methylene chloride. This may be done by
transferring the extract to a 1.0-mL volumetric and filling to the volume
mark.
NOTE: Other types of evaporation/concentration equipment maybe used,
as long as all QC requirements in Section 9 are met.
11.5 Fill the sample bottle to the volume mark noted in Sectionl 1.3.1 with tap water.
Transfer the tap water to a 1000 mL graduated cylinder, and measure the sample
volume to the nearest 10 mL. Record this volume for later analyte concentration
calculations. As an alternative to this process, the sample volume maybe
determined by the difference in weight between the full bottle (before extraction)
and the empty bottle (after extraction). Assume a sample density of 1.0 g/mL.
11.6 Analyze an aliquot of the sample extract with the GC/MS/MS system under the
same conditions used for the initial and continuing calibrations.
11.7 At the conclusion of data acquisition, use the same software that was used in the
calibration procedure to identify peaks in predetermined retention time windows of
interest. Use the data system software to examine the ion abundances of
components of the chromatogram.
11.8 IDENTIFICATION OF ANALYTES IN TANDEM MASS SPECTROMETRY --
Identify a sample component by comparison of its product ion spectrum to a
reference spectrum in the user-created data base. The GC retention time of a method
analyte should be within 1-2 sec of the retention time observed for that same
compound in the most recently analyzed CCC standard. Very early eluting
compounds may exhibit more variability in retention time. Ideally, the width of the
retention time window should be based upon measurements of actual retention time
variations of standards over the course of a day. Three times the standard deviation
of a retention time can be used to calculate a suggested window size for an analyte.
However, the experience of the analyst should weigh heavily in the interpretation of
the chromatogram.
11.8.1 In general, all ions that are present above 30% relative abundance in the
product ion mass spectrum of the standard should be present in the mass
spectrum of the sample component and should agree within an
521-30
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absolute 20%. For example, if an ion has a relative abundance of 30% in
the product spectrum of the standard, its abundance in the sample product
spectrum should be in the range of 10 to 50%. If the instrument parameters
have been set as described in Section 10.2.1.8, the precursor ion will have a
low relative abundance, and is not used as part of the analyte identification
criteria.
12. DATA ANALYSIS AND CALCULATIONS
12.1 Complete chromatographic resolution is not necessary for accurate and precise
measurements of analyte concentrations using MS/MS. In validating this method,
concentrations were calculated by measuring the product ions listed in Table 4.
Other ions may be selected at the discretion of the analyst. If the response of any
analyte exceeds the calibration range established in Section 10, dilute the extract,
add additional internal standard, and reanalyze. The resulting data should be
documented as a dilution, with an increased MRL.
12.1.1 Calculate analyte and surrogate concentrations, using the multipoint
calibration established in Section 10. Do not use daily calibration verification
data to quantitate analytes in samples. Adjust final analyte concentrations to
reflect the actual sample volume determined in Section 11.5.
12.1.2 Calculations must utilize all available digits of precision, but final reported
concentrations should be rounded to an appropriate number of significant
figures (one digit of uncertainty), typically two, and not more than three
significant figures.
NOTE: Some data in Section 17 of this method are reported with more than
2 significant figures. This is done to better illustrate the method
performance data.
13. METHOD PERFORMANCE
13.1 PRECISION, ACCURACY AND DLs -- Single laboratory DLs and LCMRLs are
presented in Table 1. Single laboratory accuracy and precision data from both
fortified reagent water and fortified matrices are presented in Tables 6 and 7. These
data were obtained on a Varian Saturn 4 GC/MS/MS system, operated in the CI
mode, using methanol as the CI reagent. Methanol was selected as the solvent used
for the method demonstration data, since it can be more widely used in both new and
vintage instrumentation. Acetonitrile can be used only in newer instruments.
Consult the instrument manufacturer for liquid CI reagent choices.
13.2 EVALUATION OF ADDITIONAL NITROSAMINES -- N-Nitrosomorpholine was
evaluated for inclusion into this method. It was not included in this method because
of unresolved problems with background contamination.
521-31
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13.3 ANALYTE STABILITY STUDIES
13.3.1 AQUEOUS SAMPLES -- Chlorinated drinking water samples, from a
surface water source, were fortified with method analytes, and preserved
and stored as required in Section 8. The average of replicate analyses (N=7)
conducted on day 0, and at three additional time points up to and beyond
14 days are presented in Figure 1. These data document the 14 day holding
time.
13.3.2 EXTRACTS — Extracts from the first day of the holding time study
described above were stored protected from light, at -15 °C, and analyzed in
replicate (N=7) on day 0, and at six additional time points up to and beyond
28 days. The results of these analyses that document the 28 day holding
time are presented in Figure 2.
13.4 SECOND LABORATORY DEMONSTRATION -- The performance of this method
was demonstrated by a second laboratory, with results similar to those reported in
Section 17. The authors wish to acknowledge the work of Mr. Ed Price and Mr.
Mark Domino of Shaw Environmental Incorporated for their participation in the
second laboratory demonstration.
14. POLLUTION PREVENTION
14.1 This method utilizes SPE technology to remove the analytes from water. It requires
the use of very small volumes of organic solvent and very small quantities of pure
analytes, thereby minimizing the potential hazards to both the analyst and the
environment when compared with the use of large volumes of organic solvents in
conventional liquid-liquid extractions.
14.2 For information about pollution prevention that may be applicable to laboratory
operations, consult "Less Is Better: Guide to Minimizing Waste in Laboratories"
available from the American Chemical Society, on-line at
http ://membership. acs. org/c/ccs/pub_9 .htm.
15. WASTE MANAGEMENT
15.1 The analytical procedures described in this method generate relatively small amounts
of waste since only small amounts of reagents and solvents are used. The only
matrix of concern is finished drinking water. However, the Agency requires that
laboratory waste management practices be conducted consistent with all applicable
rules and regulations, and that laboratories protect the air, water, and land by
minimizing and controlling all releases from fume hoods and bench operations.
Also, compliance is required with any sewage discharge permits and regulations,
particularly the hazardous waste identification rules and land disposal restrictions.
521-32
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16. REFERENCES
1. "Statistical Protocol for the Determination of the Single-Laboratory Lowest Concentration
Minimum Reporting Level (LCMRL) and Validation of the Minimum Reporting Level (MRL),"
available at www.epa.gov/OGWDW/methods/sourcalt.html.
2. Glaser, J.A., D.L. Foerst, G.D. McKee, S.A. Quave, and W.L. Budde, "Trace Analyses for
Wastewaters", Environ. Sci. Techno!.. 15 (1981) 1426-1435.
3. Wilczak, A., et al, "Formation of NDMA in Chloraminated Water Coagulated with Dadmac
Cationic Polymer", J. AWWA, 95 (2003) 94-106.
4. Lijinsky, W., "Chemistry and Biology of N-Nitroso Compounds", Cambridge University
Press, Cambridge, UK, 1992.
5. Preussmann, R, and B.W. Stewart, "N-Nitroso carcinogens, in: C.E. Searle (ed.), "Chemical
Carcinogens, American Chemical Society Monograph No. 182", (1984) 643-828.
6. "Carcinogens - Working With Carcinogens," Department of Health, Education, and Welfare,
Public Health Service, Center for Disease Control, National Institute for Occupational Safety and
Health, Publication No. 77-206, Aug. 1977.
7. "OSHA Safety and Health Standards, General Industry," (29CFR1910), Occupational Safety
and Health Administration, OSHA, (Revised, July 1, 2001).
8. "Safety in Academic Chemistry Laboratories," American Chemical Society Publication,
Committee on Chemical Safety, 6th Edition, available from the ACS Office of Society Services
by e-mail at OSS@acs.org.
9. Anspec of Ohio, 12 W. Selby Blvd., Ste. 4, Columbus, OH; telephone 1-800-521-1720.
10. Engewald, W., J. Teske, and J. Efer, "Programmed temperature vaporiser-based injection in
capillary gas chromatography", Journal of Chromatography A. 856 (1999) 259-278.
11. Mol, H.G.J., M. Althuizen, H. Janssen, C.A. Cramer and U. Brinkman, "Environmental
Applications of Large Volume Injection in Capillary GC Using PTV Injectors", J. High Resol.
Chromatogr., 19 (1996) 69-79.
12. "Large Volume sample introduction using programmed-temperature injection systems",
Chromatography Technical Notes No 11, AT AS International BV, http://atasgl.in2it.nl/ap-
note/TECHNNO_l l.pdf, accessed June 21, 2004.
521-33
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17. TABLES. DIAGRAMS. FLOWCHARTS. AND VALIDATION DATA
Table 1. Detection Limits and Lowest Concentration Minimum Reporting Levels a'b'c
Analyte
NDMA
NMEA
NDEA
NPYR
NDPA
NPIP
NDBA
DL (ng/L)
0.28
0.28
0.26
0.35
0.32
0.66
0.36
LCMRL (ng/L)
1.6
1.5
2.1
1.4
1.2
1.4
1.4
a. DLs determination from LFBs fortified at 1.0 ng/L (N = 8).
b. LCMRLs determined from LFBs fortified at 1.0, 2.0, 3.0, and 4.0 ng/L (N = 5 or 6 at each
concentration).
c. DL and LCMRL data were obtained on a Varian Saturn 4 GC/MS/MS.
521-34
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Table 2a. Chemical lonization Parameters for a Varian Saturn 4 GC/MS/MS Using
Methanol as the CI Reagent
Automatic Reaction Control (ARC)
ionization time (|_isec)
CI maximum ionization time (|_isec)
CI maximum reaction time (|_isec)
CI ion storage level (m/z)
Reagent ion eject amplitude (V)
CI reaction storage level (m/z)
CI background mass (m/z)
Emission current (|j,amps)
Electron Multiplier offset (V)
100
2000
100
20
10
15
45
50
+100
Table 2b. Chemical lonization Parameters for a Varian Saturn 2000 GC/MS/MS Using
Methanol or Acetonitrile as the CI Reagent
CI storage level (m/z)
Ejection amplitude (m/z)
Background mass (m/z)
Maximum ionization time (|_isec)
Maximum reaction time (|_isec)
Target total ion current (TIC) (counts)
Prescan lonization time (|_isec)
Emission current (|j,amps)
Electron Multiplier offset (V)
15-19
10-15
40
2000
100-120
5000
100-200
50
+300
521-35
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Table 3. Chromatographic Conditions including LVI Using a PTV Injector
Injector Temperature program
Varian Saturn 4
Temp (°C)
37
250
250
Rate
(°C/min)
0
100
0
Time (min)
0.72
2.13
40
Varian Saturn 2000
Temp (°C)
37
250
250
Rate
(°C/min)
0
100
0
Time (min)
0.6
2.13
23.00
Injector Split Vent Program
Varian Saturn 4
Time (min)
0
0.70
2.00
Split status
open"
closed
opena
Varian Saturn 2000
Time (min)
0
0.6
3.5
Split status
openb
closed
open0
a. split flow 100 mL/min
b. split ratio 25
c. split ratio 100
GC Oven Temperature Program
Varian Saturn 4
Temp (°C)
40
170
250
Rate
(°C/min)
0
4.0
20.0
Hold Time
(min)
3.0
0
3.0
Varian Saturn 2000
Temp (°C)
35
130
280
Rate
(°C/min)
0
4.0
40
Hold Time
(min)
4.0
0
0.5
521-36
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Table 4. Retention Times and Suggested Product Ions for Quantitation of Method
Analytes in Tandem Mass Spectrometry (MS/MS) Mode "b
Analyte
NDMA
NMEA
NDEA
NPYR
NDPA
NPIP
NDBA
NDMA-d6 (surrogate)
NDEA-dlO (internal standard)0
NDPA-dl4 (internal standard) c
Retention
Time (min)
8.43
11.76
14.80
22.34
22.40
24.25
30.09
8.34
14.63
22.07
Precursor
Ion (m/z)
75
89
103
101
131
115
159
81
113
145
Product Ion/
Quantitation Ion (m/z)
43 (56)
61 (61)
75 (75)
55 (55)
89 (89)
69 (69)
57 (103)
46 (59)
81(81)
97 (97)
a. Retention times obtained on Saturn 4 GC/MS/MS with the GC column and conditions
described in Section 6.10, 6.11 and Tables 2 and 3. Absolute retention times may vary slightly
with different instruments.
b. Product ions are those obtained on a Varian Saturn 4 or Saturn 2000 GC/MS/MS using
methanol as the chemical ionization reagent gas. Ions in "( )" are product ions observed using
acetonitrile as the CI reagent on the Saturn 2000. Other product ions may be used as appropriate
when different instrumentation is used.
c. One or two internal standards maybe used. If all analytes are determined, and only one IS is
used, NDPA-dl4 is recommended. If two ISs are used, use NDEA- dlO for the surrogate and the
first three eluting analytes. Use NDPA-dl4 for the rest of the analytes.
521-37
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Table 5a. MS/MS Parameters for the Varian Saturn 4 Using Methanol as the CI Reagent
Analyte
NDMA
NDMA-d6
(surrogate)
NMEA
NDEA
NDEA-dlO
(internal
standard)
NDPA-dl4
(internal
standard)
NPYR
NDPA
NPIP
NDBA
Segment #
1
1
2
3
3
4
5
5
6
7
Retention
Time Window
(min)
7.00-10.00
7.00-10.00
10.00-13.00
13.00-15.50
13.00-15.50
15.50-22.17
22.17-23.48
22.17-23.48
23.48-25.74
25.74-32.74
Scan
range
(m/z)
40-83
40-83
40-91
39-114
39-114
48-147
40-133
40-133
39-117
55-161
Scan rate
(sec/scan)
0.37
0.37
0.57
0.39
0.39
0.62
0.42
0.42
0.60
0.62
CAD
Amplitude
(volts)
0.56
0.50
0.56
0.46
0.36
0.46
0.44
0.44
0.44
0.44
CADrf
(m/z)
35.0
35.0
35.0
35.0
35.0
35.0
35.0
35.0
35.0
35.0
CAD
Time
(msec)
10
10
10
10
10
10
10
10
10
10
Precursor
Ion
Isolation
Time (msec)
2
2
2
2
2
2
2
2
2
2
Waveform type- Resonant; Default values for all other MS/MS parameters: Isolation window 3 amu, Low (DAC) offset 6 steps, High
(DAC) offset 6 steps, Broadband amplitude 10 V, Modulation range 2 steps, Modulation rate 3000 |_isec/step, Bandwidth 0 Hertz,
Ejection Amplitude 20 V; lonization RF 48 m/z
521-38
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Table 5b. MS/MS Parameters for the Varian Saturn 2000 Using Methanol as the CI Reagent
Analyte
NDMA
NDMA-d6
(surrogate)
NMEA
NDEA
NDEA-dlO
(internal
standard)
NDPA-dl4
(internal
standard)
NPYR
NDPA
NPIP
NDBA
Segment
#
1
1
2
3
3
4
5
5
6
7
Retention
Time Window
(min)
8.00-12.00
8.00-12.00
12.00-15.00
15.00-18.00
15.00-18.00
18.00-23.21
23.21-25.00
23.21-25.00
25.00-29.00
29.00-32.00
Scan
range
(m/z)
40-83
40-83
40-91
39-114
39-114
48-147
40-133
40-133
39-117
55-161
Scan rate
(sec/scan)
0.61
0.61
0.55
0.62
0.62
0.56
0.56
0.56
0.54
0.57
Excitation
Amplitude
(volts)
0.50
0.50
0.55
0.46
0.44
0.48
0.44
0.44
0.42
0.40
Excitation
Storage
Level (m/z)
35.0
35.0
35.0
35.0
35.0
48.0
35.0
35.0
35.0
35.0
Excitation
Time
(msec)
10
10
10
10
10
10
10
10
10
10
Precursor
Ion Isolation
Time (msec)
2
2
2
2
2
2
2
2
2
2
Waveform type- Resonant; Default values for all other MS/MS parameters: Isolation window 3 amu, Low
edge offset 2 steps, High edge amplitude 30 V, Modulation range 2 steps, Modulation rate 3000 |_isec/step,
frequency offset 0 Hertz, Ejection Amplitude 20 V; lonization RF 48 m/z
edge offset 6 steps, High
# of Frequencies 1, CAD
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Table 5c. MS/MS Parameters for the Varian Saturn 2000 Using Acetonitrile as the CI Reagent
Analyte
NDMA
NDMA-d6
(surrogate)
NMEA
NDEA
NDEA-dlO
(internal
standard)
NDPA-dl4
(internal
standard)
NPYR
NDPA
NPIP
NDBA
Segment
#
1
1
2
3
3
4
5
5
6
7
Retention
Time Window
(min)
8.00-12.00
8.00-12.00
12.00-15.00
15.00-18.00
15.00-18.00
18.00-23.21
23.21-25.00
23.21-25.00
25.00-29.00
29.00-32.00
Scan
range
(m/z)
40-83
40-83
40-91
39-114
39-114
48-147
40-133
40-133
39-117
55-161
Scan rate
(sec/scan)
0.61
0.61
0.55
0.62
0.62
0.56
0.56
0.56
0.54
0.57
Excitation
Amplitude
(volts)
0.50
0.50
0.55
0.46
0.44
0.48
0.44
0.44
0.42
0.40
Excitation
Storage
Level (m/z)
35.0
35.0
40.0
40.0
40.0
40.0
40.0
40.0
40.0
40.0
Excitation
Time
(msec)
10
10
10
10
10
10
10
10
10
10
Precursor
Ion Isolation
Time (msec)
2
2
2
2
2
2
2
2
2
2
Waveform type- Resonant; Default values for all other MS/MS parameters: Isolation window 3 amu, Low
edge offset 2 steps, High edge amplitude 30 V, Modulation range 2 steps, Modulation rate 3000 |_isec/step,
frequency offset 0 Hertz, Ejection Amplitude 20 V; lonization RF 48 m/z
edge offset 6 steps, High
# of Frequencies 1, CAD
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Table 6. Precision and Accuracy Data Obtained from Fortified Reagent Water at Four Concentrations
Analyte
NDMA
NMEA
NDEA
NPYR
NDPA
NPIP
NDBA
NDMA-d6
(surrogate)
Fortified Concentration
2.0 ng/L (N=7)
Accuracy
(% rec)
94.7
81.8
84.6
92.6
81.7
98.3
85.2
83.5
Precision
(RSD)
12
9.6
9.0
12
8.0
20
16
7.3
Fortified Concentration
4.0 ng/L (N=6)
Accuracy
(% rec)
92.7
83.1
92.0
102
87.6
86.3
82.2
86.0
Precision
(RSD)
11
6.3
14
4.0
7.3
6.1
7.7
7.5
Fortified Concentration
10.0 ng/L (N=4)
Accuracy
(% rec)
88.7
86.5
87.5
101
97.0
91.8
86.4
86.8
Precision
(RSD)
3.8
4.5
9.1
5.0
10
3.7
9.4
4.0
Fortified Concentration
20.0 ng/L (N=6)
Accuracy
(% rec)
89.5
90.9
95.6
101
87.1
93.6
104
88.7
Precision
(RSD)
7.8
6.9
11
6.1
7.7
4.0
8.7
8.3
Fortified samples at 2.0 and 10.0 ng/L were analyzed using a single IS (NDPA-dl4). Fortified samples at 4.0 and 20.0 ng/L were
analyzed using two internal standards (NDEA-dlO and NDPA-14).
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Table 7. Precision and Accuracy Data Obtained from Fortified Drinking Water Matrices Fortified at 20 ng/L
N=6 for each matrix
Analyte
NDMA
NMEA
NDEA
NPYR
NDPA
NPIP
NDBA
NDMA-d6
(surrogate)
Surface Water a
Accuracy
(% recovery)
85.0
81.9
88.4
85.2
77.1
81.6
79.7
82.9
Precision
(RSD)
6.6
6.2
6.5
6.5
3.7
6.7
7.2
8.4
Ground Water b
Accuracy
(% recovery)
90.8
91.0
92.8
92.7
85.1
87.3
97.8
91.5
Precision
(RSD)
4.4
7.2
7.8
4.4
6.6
2.0
2.9
8.2
High TOC Water c
Accuracy
(% recovery)
83.7
81.4
86.1
88.4
78.3
80.6
86.2
77.2
Precision
(RSD)
6.8
4.5
11.3
6.6
10.2
6.0
7.8
5.5
a. Chlorinated drinking water from a river water source.
b. Chlorinated drinking water from a ground water source. Hardness = 400 mg/L as calcium carbonate.
c. Chlorinated drinking water from a high TOC surface water source. TOC = 14 mg/L.
521-42
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Table 8. Initial Demonstration of Capability (IDC) Requirements (Summary)
Method Ref.
Sect. 9.2.1
Sect. 9.2.2
Sect. 9.2.3
Sect. 9.2.4
Sect. 9.2.5
Sect. 9.3 and
9.11
Requirement
Initial Demonstration of
Low Method
Background
Initial Demonstration of
Precision (IDP)
Initial Demonstration of
Accuracy (IDA)
Minimum Reporting
Level (MRL)
Confirmation
Detection Limit
(DL) Determination
(optional)
Quality Control Sample
(QCS)
Specification and Frequency
Analyze LRB prior to any other IDC steps, or
anytime a new lot of SPE materials or
reagents are used.
Analyze 4-7 replicate LFBs fortified at 10-20
ng/L, or other mid-range concentration.
Calculate average recovery for replicates
used in IDP
Fortify, extract and analyze 7 replicate LFBs
at the proposed MRL. Use the equation
provided to verify the MRL. Repeat after
major instrument or operational changes.
Over a period of three days, prepare a
minimum of 7 replicate LFBs fortified at a
concentration estimated to be near the DL.
Analyze the replicates through all steps of the
analysis. Calculate the DL using the equation
in Section9.2.5.
Analyze a standard from a second source, as
part of IDC, or immediately after completion
of IDC.
Acceptance Criteria
Demonstrate that all target analytes are
< 1/3 the MRL, and that possible interferences from
extraction media do not prevent the identification
and
quantification of method analytes.
RSD must be <20% for all analytes.
Mean recovery 70-130% of true value.
See Section 9.2.4 for confirmation criteria.
NOTE: Data from DL replicates are not required to
meet method precision and accuracy criteria. If the
DL replicates are fortified at a low enough
concentration, it is likely that they will not meet
precision and accuracy criteria.
If analyzed as a calibration sample, CCC criteria
apply. If analyzed as an LFB, those criteria apply.
521-43
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Table 9. Quality Control Requirements (Summary)
Method Ref.
Requirement
Specification and Frequency
Acceptance Criteria
Sect. 8.1 -
Sect 8.4
Sample Collection,
Preservation, and
Holding Time
14 days, protected from light, with addition
of sodium thiosulfate.
Iced or refrigerated at 10° C or less for up to 48
hours to allow time for shipping; refrigerated at 6° C
or less, after arrival at the laboratory.
Sect. 8.4
Extract Holding Time
28 days
Stored at -15° C or less in amber vials. Protect from
light.
Sect 9.4
Laboratory Reagent
Blank (LRB)
One with each extraction batch of up to 20
field samples.
Demonstrate that all target analytes are
< 1/3 the MRL, and that possible interferences from
extraction media or reagents do not prevent the
identification and quantification of method analytes.
Sect. 9.6
Laboratory Fortified
Blanks (LFB)
Analyze at least one LFB daily or one for
each extraction batch of up to 20 field
samples. Rotate the fortified concentration
between low, medium and high amounts.
Results of LFB analyses must be 70-130% of the
true value for each analyte and surrogate for all
fortified concentrations greater than the lowest CAL
point. Results of LFBs corresponding to the lowest
CAL point must be 50-150% of the true value.
Sect. 9.7
Internal Standard
At least one internal standard is added to all
calibration standards and extracts.
Peak area counts for the IS in LFBs, LRBs and
sample extracts must be within 70-130% of the peak
area in the most recent CCC, and 50-150% of
average area in the initial calibration.
Sect. 9.8
Surrogate Standards
Surrogate standard is added to all calibration
standards, samples, LFBs, LFSMs, LFSMDs,
FDs, and LRBs.
Recovery for the surrogate in all calibration
standards, LRB, LFB, LFSM, LFSMDs, FD and
sample extracts must be 70-130% of the true value.
521-44
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Method Ref.
Requirement
Specification and Frequency
Acceptance Criteria
Sect. 9.9
Laboratory Fortified
Sample Matrix (LFSM)
Analyze one LFSM per extraction batch (20
field samples or less) fortified with method
analytes at a concentration > the native
concentration.
Recoveries not within 70-130% of the fortified
amount may indicate a matrix effect.
Sect. 9.10
Field Duplicates or
Laboratory Fortified
Sample Matrix
Duplicates (LFSMD)
Analyze 1 FD for each 20 samples, or 1 per
extraction batch, whichever is greater. See
the referenced Section for a discussion of
when LFSMDs should be analyzed.
Suggested RPD <30%.
Sect. 9.11
Quality Control Sample
(QCS)
Analyze QCS whenever new standards are
prepared, or at least quarterly.
If analyzed as a calibration sample, CCC criteria
apply. If analyzed as an LFB, those criteria apply.
Sect. 10.2.
Initial Calibration
Use internal standard calibration technique to
generate an average RF, or first or second
order calibration curve for each analyte. Use
a minimum of 3 standards for a calibration
range of 1 order of magnitude, and at least 5
standards for 2 orders of magnitude.
When each calibration standard is calculated as an
unknown using the calibration curve, the result must
be 70-130% of the true value for all but the lowest
standard. The lowest standard must be 50-150% of
the true value.
Sect. 10.3
Continuing Calibration
Check
Verify initial calibration by analyzing a
calibration standard prior to analyzing
samples, after every 10 samples, and after the
last sample. Always analyze a low
concentration (near the MRL) CCC at the
beginning of the analysis period. Rotate
through low, medium, and high
concentration calibration standards to meet
the CCC for every 10 samples requirement.
The result for each analyte and surrogate must be
70-130% of the true value for all concentrations
except the lowest CAL point for each analyte. The
lowest CAL point for each analyte must be 50-150%
of the true value.
The peak area of the IS must be within 70-130% of
the peak area in the most recent CCC, and 50-150%
of the average peak area calculated during initial
calibration.
521-45
-------�
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521-46
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521-47
-------� |